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Impact of physicochemical properties of DNA/PEI complexes on transient transfection of mammalian cells

机译:DNA / PEI复合物物理化学性质对哺乳动物细胞瞬时转染的影响

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Polyethyleneimine (PEI) has been used extensively for transient gene expression (TGE) in mammalian cell cultures. However, the relationship between DNA/PEI complex preparation and their biological activity has not been fully established. Here, a systematic study of DNA/PEI complexes, their physicochemical properties during formation and their transfection efficiency was performed on a virus-like particle (VLP) production platform. The same chemically defined cell culture medium for DNA/PEI complex formation was used as an alternative to simple ionic solutions to minimize changes in complex properties during transfection. Upon formation, an initial concentration of 1E+ 10 DNA/PEI complexes/mL underwent partial aggregation with an average size of 300 nm. The participation of NaCl ions in the evolution of complexes was analyzed by X-ray spectroscopy, stressing the relevance of complexing media composition in TGE strategies. After 15 min incubation, 250 complexes plus aggregates per cell were estimated at the time of transfection. Such heterogeneous preparations cannot be easily characterized; subsequently, nanoparticle tracking analysis (NTA) and cryo-electron microscopy were combined to achieve a complete picture of the preparation. Finally, the contribution of each DNA/PEI complex subpopulation was tested by drug inhibition endocytosis. Interestingly, all complexes delivered DNA efficiently and high size aggregates, which enter through macropinocytosis, when inhibited presented a major contribution to transfection efficiency. There is a need to understand the physicochemical factors that participate in DNA delivery protocols. Hence, this study provides new insights into the characterization of DNA/PEI complexes that will assist in more productive and reproducible TGE strategies.
机译:聚乙烯亚胺(PEI)已广泛用于哺乳动物细胞培养物中的瞬时基因表达(TGE)。然而,DNA / PEI复合物制剂与其生物活性之间的关系尚未完全建立。这里,对形成期间的DNA / PEI复合物的系统研究及其转染效率在病毒样颗粒(VLP)生产平台上进行。用于DNA / PEI复合物形成的相同化学定义的细胞培养基作为简单的离子溶液的替代方案,以最小化转染过程中复杂性能的变化。在形成后,初始浓度为1E + 10DNA / PEI复合物/ mL,平均尺寸为300nm的部分聚集。通过X射线光谱分析NaCl离子在复合物的演变中的参与,施加络合培养基组合物在TGE策略中的相关性。孵育15分钟后,在转染时估计每种细胞的250个络合物加上聚集体。这种非均相制剂不能容易地表征;随后,组合纳米粒子跟踪分析(NTA)和冷冻电子显微镜,以实现制剂的完整图像。最后,通过药物抑制内吞作用测试每种DNA / PEI复合亚群的贡献。有趣的是,所有复合物都有效地递送DNA,并且当抑制呈现出通过癌细胞增多作用的大尺寸聚集体赋予转染效率的主要贡献。需要了解参与DNA递送方案的物理化学因素。因此,本研究为DNA / PEI复合物的表征提供了新的见解,这些洞察力将有助于更高效和可重复的TGE策略。

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